Blocking sporulation by inhibiting spoIIE

ABSTRACT

We have shown that the control of solventogenesis and sporulation can be genetically uncoupled in  C. acetobutylicum . In strain 824(pASspo), the absence of SpoIIE causes sporulation to be blocked at stage II. The cell remains in a vegetative state, and this allows solvent production to proceed for longer and for solvents to accumulate more rapidly and to a higher concentration. The characteristic drop in OD600 observed in wild type and control strains of  C. acetobutylicum  after 48-72 hours as the cells transition from the solventogenic phase to sporulation is notably absent in the fermentations of 824(pASspo). Mutant S (wild type background, spoIIE disrupted), Mutant BS (Mutant B background, spoIIE disrupted), Mutant HS (Mutant H background, spoIIE disrupted) and Mutant bukS (buk- background, spoIIE disrupted) were generated to create stable solvent producing bacteria with complete inactivation of the SpoIIE protein. Similarity between the SpoIIE protein of  C. acetobutylicum, B. subtilis , and other  Clostridial  species indicates that the techniques used in  C. acetobutylicum  can be applied to other solvent producing  Clostridia.

PRIOR RELATED APPLICATIONS

This application claims the benefit under 35 USC §119(e) to U.S. Provisional Application Ser. No. 60/584,727 filed Jul. 1, 2004, entitled “Blocking Sporulation by Inhibiting SPOIIE,” which is incorporated herein in its entirety.

FEDERALLY SPONSORED RESEARCH STATEMENT

The present invention may have been developed with funds from the United States Government. Therefore, the United States Government may have certain rights in the invention.

REFERENCE TO MICROFICHE APPENDIX

Not applicable.

REFERENCE TO A SEQUENCE LISTING

A “Sequence Listing” with sequences labeled SEQ ID NO: 1-25 is attached hereto. A compact disc containing a Computer Readable Form (CRF) labeled “SEQUENCE LISTING.txt” is incorporated by reference. The copy in CRF is identical to the paper copy of the “Sequence Listing” submitted herewith.

FIELD OF THE INVENTION

The invention relates to the production of organic solvents in Clostridium acetobutylicum. Decreasing activity of the Stage II Sporulation Protein E (SpoIIE) increases solventogenesis in Clostridia by inhibiting sporulation without interfering with solvent production.

BACKGROUND OF THE INVENTION

The Gram-positive, obligate anaerobe C. acetobutylicum was used for the industrial production of the solvents acetone and butanol for over 60 years in the 20th century. With chemical synthesis of acetone and butanol proving significantly more economic, there are no industrial fermentation plants of C. acetobutylicum operational in the world today (11). However, over the last 20 years the genetics and biochemistry of C. acetobutylicum have been investigated in detail as we try to understand and improve upon the processes that control the production of solvents. Biological sources of organic solvents will become more economical as raw materials become more scarce or expensive and the need for renewable solvent sources increase.

Whereas much is known about the biochemistry of C. acetobutylicum metabolism and the genes and proteins that catalyze these processes, relatively little is known about the genetic control of the expression of these genes. Stage 0 Sporulation Protein A (Spo0A) controls both the onset of solventogenesis and the process of sporulation in C. beijerinckii and C. acetobutylicum (30, 20). In strain SKO1 of C. acetobutylicum, where Spo0A is deleted, acetone and butanol production is reduced to 2% and 8% of wild type levels respectively. Furthermore, SKO1 cells fail to sporulate and form extended filaments of conjoined rods (20).

Studies have also shown that there are a considerable number of Bacillus subtilis homologues in C. acetobutylicum including sigma factors and other proteins required for sporulation (32, 28). Although solventogenesis does not occur in B. subtilis, it appears that a cascade of sigma factors and stages similar to those involved in B. subtilis sporulation are present in C. acetobutylicum.

The control of solventogenesis in C. acetobutylicum is genetically linked to the control of sporulation, as shown by the Spo0A studies (30, 20). It has been suggested that solventogenesis and sporulation may be genetically uncoupled at some point during early sporulation (19), although as yet there are no reports of any attempts to do so. If solventogenesis could be genetically separated from sporulation, this would serve as an interesting and important illustration of the complexity of bacterial genetic control. Additionally, it may prove useful in bioengineering solvent producing strains of Clostridium for use in industry. A strain of C. acetobutylicum that underwent solventogenesis without entering sporulation would increase solvent production without inactivation, an ideal situation for large scale continuous fermentations.

SUMMARY OF THE INVENTION

Clostridium strains transformed with an antisense expression vector increased ethanol, acetone and butanol production by 225%, 43% and 110% respectively compared to the control strains. An antisense RNA vector targeted against spoIIE, designated pASspo was constructed and evaluated in various C. acetobutylicum strains. The genomic spoIIE gene was disrupted in C. acetobutylicum strains to generate Mutant S, Mutant BS, Mutant HS, and Mutant S buk-. These strains enable the stable production of solvents for continuous fermentation. Based on these experiments, a method of increasing solvent production was developed wherein a decrease in Clostridial SpoIIE activity inhibits sporulation while allowing continued solventogenesis, thus improving solvent yield.

As used herein Stage II Sporulation Protein E (SpoIIE) is used to refer to the spoIIE gene and SPOIIE gene product.

The term “isolated, ” as used herein, refers to a nucleic acid or polypeptide removed from its native environment. An example of an isolated protein is a protein bound by a polyclonal antibody, rinsed to remove cellular debris, and utilized without further processing. Salt-cut protein preparations, size-fractionated preparations, affinity-absorbed preparations, recombinant genes, recombinant protein, cell extracts from host cells that expressed the recombinant nucleic acid, media into which the recombinant protein has been secreted, and the like are also included. The term “isolated” is used because, for example, a protein bound to a solid support via another protein is at most 50% pure, yet isolated proteins are commonly and reliably used in the art.

The term “substantially purified, ” as used herein, refers to nucleic acid or protein sequences that are removed from their natural environment and are at least 75% pure. Preferably, at least 80, 85, or 90% purity is attained.

“Purified, ” as used herein refers to nucleic acids or polypeptides separated from their natural environment so that they are at least 95% of total nucleic acid or polypeptide in a given sample. Protein purity is assessed herein by SDS-PAGE and silver staining. Nucleic acid purity is assessed by agarose gel electrophoresis and EtBr staining.

The phrases “nucleic acid” or “nucleic acid sequence, ” as used herein, refers to polynucleotides, which may be cDNA or RNA and which may be single-stranded or double-stranded. The term also includes peptide nucleic acid (PNA), or to any chemically DNA-like or RNA-like material. “cDNA” refers to copy DNA made from mRNA that is naturally occurring in a cell. Combinations of the same are also possible (i.e. , a recombinant nucleic acid that is part gDNA and part cDNA).

The term “oligonucleotide, ” as used herein, refers to a nucleic acid sequence of at least about 15 nucleotides to 100 nucleotides, and all integers between. Preferably, oligonucleotides are about 21 to 81 nucleotides, and most preferably about 51 to 78 nucleotides. Generally, an oligonucleotide must be greater than 21 to 27 nucleotides long for specificity, although shorter oligonucleotides will suffice in certain applications.

The term “antisense, ” as used herein, is a nucleic acid sequence complementary to a segment of genetic material (as MRNA) and serving to inhibit gene function. Antisense oligonucleotides can inhibit either transcription or translation and can be synthesized to include non-natural nucleotides. Furthermore, an antisense oligonucleotide can be recombinantly incorporated into a genomic, viral, or plasmid DNA and operably linked to a promoter for expression of the antisense oligonucleotide in vivo.

The terms “operably associated” or “operably linked, ” as used herein, refer to functionally coupled nucleic acid sequences.

The terms “disruption” and “disruption strains, ” as used herein, refer to cell strains in which the native gene is mutated, deleted, or interrupted in such a way as to decrease the activity of the protein.

“Reduced activity” of the SpoIIE protein is defined herein to be that reduction sufficient to inhibit sporulation. In a preferred embodiment, the reduction in activity is at least 75% as compared with control bacteria. Preferably, at least 80, 85, or 90% reduction in activity is attained. Use of a frame shift mutation, early stop codon, point mutations of critical residues, or deletions or insertions can completely inactivate (100%) gene product by completely preventing transcription and/or translation of active protein.

Alignments were performed using BLAST homology alignment as described by Tatusova & Madden (37) and available online at www.ncbi.nlm.nih.gov/BLAST/. The default parameters were used, except the filters were turned OFF. As of Jan. 1, 2001 the default parameters were as follows: BLASTN or BLASTP as appropriate; Matrix=none for BLASTN, BLOSUM62 for BLASTP; G Cost to open gap default=5 for nucleotides, 11 for proteins; E Cost to extend gap [Integer] default=2 for nucleotides, 1 for proteins; q Penalty for nucleotide mismatch [Integer] default=−3; r reward for nucleotide match [Integer] default=1; e expect value [Real] default=10; W wordsize [Integer] default=11 for nucleotides, 3 for proteins; y Dropoff (X) for blast extensions in bits (default if zero) default=20 for blastn, 7 for other programs; X dropoff value for gapped alignment (in bits) 30 for blastn, 15 for other programs; Z final X dropoff value for gapped alignment (in bits) 50 for blastn, 25 for other programs.

Abbreviations: Ap^(R), ampicillin resistance cassette; cat, promoterless chloramphenicol acetyl transferase gene; catP, chloramphenicol acetyl transferase open reading frame with complete promoter; Thi^(R)/Cm^(R), thiamphenicol/chloramphenicol resistance cassette with functional catP; MLS^(R), macrolide, lincosamide and streptogramin A resistance cassette; Str^(R), streptomycin resistance cassette; Ap, ampicillin; Em, erythromycin; Km, kanamycin; Cm, chloramphenicol; ColE1, Gram-negative origin of replication; OriII, repL, Gram-positive origin of replication; lacZ, promoterless β-galactosidase gene derived from Thermoanaerobacterium thermosulfurogenes EM1 (38); lacZ′, truncated, non-finctional copy of lacZ; mcrA, ΔmcrBC, methylcytosine-specific restriction system abolished; recA1, homologous recombination abolished; Spo0A⁻, deletion of Spo0A. Common restriction enzymes and restriction sites can be found at NEB® (NEW ENGLAND BIOLABS®, www.neb.com) and INVITROGEN® (www.invitrogen.com). ATCC®, AMERICAN TYPE CULTURE COLLECTION™(www.atcc.org).

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1. Antisense construct to spoIIE. The spoIIE antisense construct consists of oligonucleotide “spoasastop” (SEQ ID NO: 22) and “spoasbtm” (SEQ ID NO: 23). The single underlined GATC forms the 5′ BamHI “sticky” end. The black shaded region includes 38 bases of the spoIIE open reading frame, followed by 16 bases of the upstream leader sequence, shaded dark gray. The bold region forms the 17 base rho-independent terminator region from an antisense RNA targeted against the glnA gene, found naturally in Clostridium saccharobutylicum NCP262 (10).

FIG. 2. CAT activity in strain 824(pCATspo) (▪) and control strain 824(pCATP) (□). The solvent levels are shown for acetone (▴) and butanol (♦). Data are shown ±1 standard error. For acetone and butanol, n=9; for 824(pCATP) CAT activity, n=3; for 824(pCATspo) CAT activity, n=6.

FIG. 3. β-galactosidase activity in strain 824(pTLspo) (♦) and control strains 824(pThilac) (⋄), SK(pThilac) (□) and SK(pTLspo) (▪). Data are shown ±1 standard error. For 824(pThilac), 824(pTLspo) and SK(pTLspo), n=4; for SK(pThilac), n=3.

FIG. 4. Growth and product formation fermentations of strain 824(pASspo) (▪) and strain 824(pASsos) (□). The name for each profile of and is shown above each graph. Data are shown ±1 standard error. For each data point, n=4.

FIG. 5. Phylogenetic tree of SpoIIE in different bacterial species. SpoIIE homologues shown are the 11 most identical to SpoIIE in C. acetobutylicum, as identified in a BLAST search of known bacterial genomes. Phylogenetic tree was generated using the PHYLIP™ format. Both BLAST and PHYLIP™ tools are available on the BIOLOGYWORKBENCH™, located at workbench.sdsc.edu/ (San Diego Supercomputer Center, University of California—San Diego, Calif. ).

FIG. 6. Hydropathy plot of SpoIIE. Hydropathy plots N-terminal region of SpoIIE from B. subtilis (gray line & X-axis scale) and C. acetobutylicum (black line & X-axis scale). Gray “▾” symbols at top of graph indicate transmembrane domains identified in SpoIIE of B. subtilis (2).

FIG. 7. Amino acid sequence alignment of SpoIIE in B. subtilis and C. acetobutylicum. Alignment was performed on the C-terminal amino acids of SpoIIE in B. subtilis (GENBANK® Acc. # P37475) and C. acetobutylicum (GENBANK® Acc. # NP 349801) using the CLUSTALW tool of the Biology Workbench (San Diego Supercomputer Center, University of California—San Diego, Calif. ). Numbers indicate amino acid position. Background shading black=conserved residue; dark gray=conserved property; white background=no consensus. (28). Black “▾” symbols indicate the invariant D610, D628, D746, G747 and D795 in B. subtilis. Common motifs around the invariant D746, G747 and D795 are shown in boxes (9, 1).

FIG. 8. Acid/solvent production in 120 hour 824(pMspo) fermentations. Graphs for 120 hour fermentations of strains 824(pIMPl), 824(pMspoD) and 824(pMspo). The data for 824(pMspo) are therefore divided into those cultures which produced solvents, designated 824(pMspo)+, and those which did not, designated 824(pMspo)0. The data is arranged to allow comparison of growth and acid/solvent production between the 4 data sets as follows; A. Optical density (600 nm), B. Ethanol production, C. Acetone production, D. Acetate production, E. Butanol production, F. Butyrate production. All data points are shown ±1 standard error. For 824(pIMP1), 824(pMspoD) and 824(pMspo)+, n=4; for 824(pMspo)0, n=3.

DESCRIPTION OF EMBODIMENTS OF THE INVENTION

Methods for producing organic solvents are disclosed, one example of which is reducing SpoIIE activity in a solvent producing strain of Clostridium sufficiently to inhibit sporulation, culturing said strain under conditions suitable for solventogenesis, and purifying the solvents from the culture media.

Also provided are recombinant solvent producing Clostridia that have reduced SpoIIE protein activity sufficient to inhibit sporulation. Activity can be reduced 75%, 80%, 85%, 90%, or 95%. In a preferred embodiment the activity is reduced to essential nil. Such recombinant Clostridium can be engineered to produce antisense nucleotides to inhibit SpoIIE expression, or can be provided with SpoIIE mutations sufficient to inhibit activity. The mutations can be changes in the regulatory regions, premature stop codons, frame shift mutations, large insertions or deletions, or point mutations of invariant residues, but in an preferred embodiment, the mutation is a knock-out. Other methods of inhibiting SpoIIE activity can also be used.

Also provided are antisense oligonucleotides that ftnction to decrease SpoIIE activity sufficiently to inhibit sporulation, without decreasing solventogenesis. Some examples are oligonucleotides comprising SEQ ID NO: 22, 23, 24, or 25. Also provided are mutant spoIIE gene sequences that can be used to create knock-strains or mutations that can be used to otherwise reduce SpoIIE activity.

Escherichia coli was grown in Luria-Bertani (LB) medium aerobically at 37° C. (26) appropriately supplemented with Ap at 100 μg/ml, Em at 200 μg/ml, Km at 50 μg/ml or Cm at 35 μg/ml. Strains were stored at −80° C. in medium supplemented with 50% glycerol. C. acetobutylicum strains were grown anaerobically in Clostridial Growth Medium (CGM) at 37° C. (21) appropriately supplemented with Em/Cm at 40 μg/ml or Thi at 25 μg/ml. Strains were stored as horse-serum supplemented lyophilized stocks at room temperature or at −80° C. in medium supplemented with 10% glycerol. For the sporulation and morphology assays, strains were grown on agar-solidified CBM supplemented with Em (40 μg/ml) anaerobically at 37° C (29).

EXAMPLE 1

Materials and Methods TABLE 1 Strains and Plasmids Strain or plasmid Relevant characteristics Reference ATCC # Strains C. acetobutylicum Wild type ATCC ® 824 C. acetobutylicum SKO1 spo0A⁻, MLS^(R) 20 E. coli DH10β mcrA, ΔmcrBC, recAl, Str^(R) NEB ™ C. acetobutylicum MutS ΔspoIIE, catP this study C. acetobutylicum MutB Mutant B (824 solR::pO1X) 27 C. acetobutylicum MutBS Mutant B ΔspoIIE, catP this study C. acetobutylicum MutH Mutant H (824 solR::pO1X) 27 C. acetobutylicum MutHS Mutant H ΔspoIIE, catP this study C. acetobutylicum M5S degenerated ΔspoIIE, catP this study C. acetobutylicum buk- Δ butyrate kinase 15 C. acetobutylicum MutS buk- Δ butyrate kinase, ΔspoIIE, catP this study Plasmids pCATP MLS^(R), OriII, ColE1ori, catP 34 pCATspo MLS^(R), OriII, ColE1ori, catP, spoIIE promoter 35 pSA12 MLS^(R), OriII, ColE1ori, lacZ' 43 pSC12lacZ Cm^(R), OriII, ColE1ori, lacZ' 43 pHT3 Ap^(R), MLS^(R), ColE1ori, repL, lacZ 38 pThilac Thi^(R), OriII, ColE1ori, lacZ 35 pTLspo Thi^(R), OriII, ColE1ori, lacZ, spoIIE promoter 35 pIMP1 Ap^(R), MLS^(R), ColE1ori, repL 24 pMspo Ap^(R), MLS^(R), ColE1ori, repL, spoIIE 35 pMspoD Ap^(R), MLS^(R), ColE1ori, repL, spoIIE' 35 pSpoΔ4 MLS^(R), OriII, ColE1ori, lacZ', spoIIE this study pSOS94 ptb promoter, Ap^(R), MLS^(R), ColE1ori, repL 38 pASsos ptb promoter, Ap^(R), MLS^(R), ColE1ori, repL 35 pASspo ptb promoter, Ap^(R), MLS^(R), ColE1ori, repL 35

Plasmids were purified from E. coli using the QIAPREP™ Miniprep protocols. DNA was purified from agarose gels using the QIAQUICK™ Gel Extraction Kit, and PCR product or enzymatically-manipulated DNA was purified using the QIAQUICK™ PCR Purification Kit (QIAGEN™ Inc. , Valencia, Calif. ). Plasmids were purified from C. acetobutylicum according to the protocol developed by Harris (18). Genomic DNA was purified from C. acetobutylicum using the PUREGENE™ Genomic DNA Purification Kit (GENTRA SYSTEMS™, Minneapolis, Minn. ).

All commercial enzymes used in this study (Taq polymerase, restriction endonucleases, calf intestinal phosphatases, T4 DNA ligase, Klenow fragment of DNA polymerase I) were used according to the manufacturers' recommendations.

Automated DNA sequencing was performed by LONESTAR™ automated DNA sequencing (LONESTAR LABORATORIES™ Inc. , Houston, Tex., www.lslabs.com).

Prior to transformation into C. acetobutylicum, E. coli plasmid DNA was methylated by the phi3TI methyltransferase to prevent restriction by the Clostridial endonuclease Cac8241 (25). This was achieved by transformation of the required plasmid into DH10β E. coli harboring vector pDHKM (43) carrying an active copy of the phi3TI methyltransferase gene. Electrotransformation of methylated plasmids into C. acetobutylicum was carried out according to a modification of the protocol developed by Mermelstein (24). Positive transformants were isolated on agar-solidified CGM supplemented with the appropriate antibiotic, and transformations were confirmed by plasmid DNA purification. TABLE 2 SEQ ID NO AND DESCRIPTION SEQ ID NO: TYPE Length Name and Description 1 DNA 2388 nt  Wild type spoIIE cDNA [NC_003030 at 3351731 . . . 3354118] 2 Peptide 795 aa   Wild type SPOIIE protein [NP_349801] 3 DNA 33 nt spoprom - spoIIE primer 4 DNA 35 nt sporev - spoIIE primer 5 DNA 42 nt spofor - spoIIE primer 6 DNA 30 nt ASseq - automated sequencing primer 7 DNA 25 nt adhEleft - adhE primer 8 DNA 25 nt adhEright - adhE primer 9 DNA 38 nt sinRfor - sinR primer 10 DNA 34 nt sinRrev - sinR primer 11 DNA 36 nt spofragUP - Upstream spoIIE primer 12 DNA 35 nt spofragDS - Downstream spoIIE primer 13 DNA 30 nt catPstN - catP primer 14 DNA 30 nt catPstC - catP primer 15 DNA 42 nt spoORFfor - spoIIE ORF primer 16 DNA 35 nt spoORFrev - spoIIE ORF primer 17 DNA 24 nt bukDfor - butyrate kinase primer 18 DNA 21 nt bukDrev - butyrate kinase primer 19 DNA 26 nt solR453 - pO1X primer, solR primer 20 DNA 23 nt Tc238 - pO1X primer 21 DNA 28 nt solR1361 - solR primer 22 DNA 77 nt spoastop - spoIIE antisense oligonucleotide 23 DNA 77 nt spoasbtm - spoIIE antisense oligonucleotide 24 DNA 54 nt spoastop' - spoIIE antisense oligonucleotide 25 DNA 54 nt spoasbtm' - spoIIE antisense oligonucleotide

All assays were conducted from single colonies of transformed C. acetobutylicum grown in closed-cap batch fermentations of 100 ml CGM supplemented with the appropriate antibiotic 37° C. in a FORMA SCIENTIFIC™ anaerobic chamber (THERMO FORMA™, Marietta, Ohio. To allow for differences in lag time following inoculation, zero hour (T0) was determined when the culture had reached an OD600 of 0.1. Fermentations were allowed to proceed for 120 hours.

EXAMPLE 2

Determining SpoIIE Expression Patterns

To investigate the role of SpoIIE in the control of solventogenesis and sporulation in C. acetobutylicum, initial studies focused on using the spoIIE promoter with a chloramphenicol acetyl-transferase (CAT) or β-galactosidase (β-Gal) reporter system to elucidate SPOIIE expression patterns. These experiments showed that spoIIE is expressed transiently in wild type C. acetobutylicum during mid- to late solventogenesis, but that there is no detectable expression of spoIIE in the spo0A-deleted mutant strain, SKO1. This agrees with reports that Sp0A is required for the transcriptional activation of spoIIE in B. subtilis (42), that spoIIE expression may be regulated by spoA, and that reduction of SPOIIE protein could be used to separate sporulation from solventogenesis.

A. CAT Assays

A chloramphenicol acetyl-transferase (CAT) reporter plasmid, pCATspo (35), was used to investigate expression patterns for the spoIIE gene in wild-type Clostridium. The pCATP plasmid (34) is the control without an spoIIE promoter construct. By operably linking the spoIIE promoter to the cat reporter protein, CAT activity in C. acetobutylicum strain 824(pCATspo) could be used to determine the expression patterns of the wild-type spoIIE gene and compare to the control strain 824(pCATP) . FIG. 2 demonstrates that CAT expression (spoIIE promoter) increases at a uniform rate between 42 and 54 hours to a maximum of approximately 14 units CAT/mg protein at 54 hours. Over the next 24 hours, the CAT activity returns to basal levels. Combined acetone and butanol concentrations from all cultures show that the individual cultures were in approximately the same stage of solventogenesis. These data show that the spoIIE promoter is active during mid- to late solventogenesis, which is the stage of growth where the cells are transitioning from vegetative growth to sporulation.

B. β-Gal Assays

A thiamphenicol-resistant lacZ reporter plasmid, pTLspo (35), was used to assay the spoIIE promoter activity in both wild-type and SKO1 (spoA-) Clostridium. Control plasmid pThilac (35) does not contain an spoIIE promoter. As with the CAT assay, fermentation products were assayed by gas chromatography to demonstrate that the individual cultures were in the same stages of solventogenesis. (data not shown). In both control strains 824(pThilac) and SK(pThilac), β-Gal activity was less than 1.2 unit/mg protein in any sample (data not shown). In strain 824(pTLspo), β-Gal activity is detectable during late solventogenesis, reaching a maximum of ˜50 units/mg protein from 66 to 78 hours growth after T0. This is approximately 12 hours later than CAT activity in 824(pCATspo). Additionally, β-Gal activity continues for over 48 hours, whereas CAT activity lasted 30 hours. These differences are a reflection of the variability in growth of C. acetobutylicum. β-Gal activity in SK(pTLspo) is not different from that observed in the control strains, and remains less than 1.3 units/mg protein in any sample indicating that spoIIE is not expressed in SKO 1.

These experiments indicate that Clostridial spoIIE expression occurs mid- to late solventogenesis, at which time the cell are expected to be transitioning between solventogenic growth and the onset of sporulation. SpoIIE expression was not observed in SKO1 (Spo0A-strain) we can conclude that, as in B. subtilis, Spo0A is required for the correct expression of spoIIE (42).

EXAMPLE 3

Product Formation with Increased SpoIIE

The SPOIIE expression vector pMspo (35) was generated to assess the effect of additional SPOIIE expression in wild-type Clostridium. The pMspo vector comprises the wild type spoIIE open reading frame including promoter. The pMspoD control plasmid (35) contains the upstream and downstream DNA (including promoter) with the open reading frame deleted. This ensures that effects seen in pMspo containing cells are not artifacts of the non-translated DNA sequences. Both constructs were generated in the Am^(R)/MLS^(R) pIMPI shuttle vector (24). C. acetobutylicum strain 824(pMspo) and the control strains 824(pIMP1) and strain 824(pMspoD) were generated by electrotransformation as described. In cultures of 824(pIMP1), 824(pMspoD) and 824(pMspo)+, product formation does not differ significantly between the strains. Acetone and butanol concentrations reach maximums of 25-27 mM and ˜70 mM, which are typical for fermentations of this scale. After 120 hours, most of the acetate and butyrate has been reassimilated into acetone and butanol, leaving final concentrations of 10-12 mM acetate and less than 5 mM of butyrate. No ethanol, acetone or butanol is produced in cultures of 824(pMspo)0. This results in the accumulation of acids, and hence acetate and butyrate levels are elevated by ˜33% and ˜400% respectively, after 120 hours growth. TABLE 3 PRODUCT FORMATION Strain Ethanol (mM) Acetone (mM) Acetate (mM) Butanol (mM) Butyrate (mM) 824 (pIMP1) 7.25 ± 0.48 24.50 ± 0.87 12.50 ± 1.32 69.75 ± 3.50 5.00 ± 0.41 824 (pMspoD) 7.00 ± 0.71 25.50 ± 1.94 11.75 ± 0.48 72.75 ± 2.93 3.50 ± 0.29 824 (pMspo)+ 7.25 ± 0.95 27.00 ± 2.12 10.50 ± 0.65 69.50 ± 4.01 3.25 ± 0.48 824 (pMspo)0 0.00 ± 0.00  0.00 ± 0.00 17.67 ± 0.88  0.00 ± 0.00 37.33 ± 2.03 

Using an α-amylase assay (35), it was determined that none of the cultures of 824(pIMP1), 824(pMspoD) and 824(pMspo)+were degenerate, but all three cultures of 824(pMspo)0 were degenerate and had lost the pSOL1 megaplasmid (7, 19, 31). This degeneration event required an intact copy of the spoIIE open reading frame, as none of the cultures of 824(pMspoD) degenerated. Thus increased levels of SPOIIE did not adversely affect solvent production but did cause degeneration of the pSOL1 megaplasmid.

EXAMPLE 5

Product Formation with SpoIIE Antisense

The antisense vector, pASspo, targeted against spoIIE was designed according to the method of Desai (10). Oligonucleotides “spoastop” (SEQ ID NO: 22) and “spoasbtm” (SEQ ID NO: 23) were diluted to a concentration of 0.5 μg/μl. 9 μl of the “top” and 9 μl of the “btm” oligonucleotide were mixed with 2 μl of 10× STE buffer (100 mM Tris-HCI, 500mM NaCl, 10 mM EDTA, pH 8. 0), and placed in a water bath set to 94° C. The water bath was allowed to cool to room temperature overnight, during which time the oligonucleotides annealed to form the antisense construct shown in FIG. 1. Vector pSOS94 (GENBANK® Acc. # AY187685) was digested with BamHI and SfoI, and the 5.0 kb fragment was purified. This fragment was treated with the Klenow fragment of DNA polymerase I and self-ligated to form the control vector pASsos. The spoIIE antisense construct and the 5.0 kb fragment of pSOS94 were BamHI cohesive-end ligated, treated with the Klenow fragment of DNA polymerase I and self-ligated to form vector pASspo. Correct construction of pASsos and pASspo was confirmed by automated sequencing using primer “ASseq” (SEQ ID NO: 6) which hybridizes to pSOS94 between 148 and 118 bases upstream of the ptb promoter.

Growth and product formation in 120 hour fermentations of strains 824(pASsos) and 824(pASspo) is shown in FIG. 4. Cultures of 824(pASspo) grew significantly better than 824(pASsos) with a maximum OD600 of ˜6.5 compared to ˜4.5. Maximum acetate concentrations in both strains were similar at ˜40 mM after 24 hours growth. However, acetate levels decrease rapidly in 824(pASspo) as acetate is reassimilated into acetone, to a minimum of ˜9 mM after 48 hours growth. Acetate production increases again after 48 hours, which coincides with acetone concentrations reaching a maximum of ˜45 mM, at which they remain for the remainder of the fermentation. This is 50% greater than maximum acetone concentrations of ˜30 mM observed in 824(pASsos) after 120 hours growth.

Butyrate production in both strains does not differ significantly, but this is not reflected in butanol production. In the control strain, butanol production follows a typical pattern, reaching a maximum of ˜66 mM after 120 hours growth. 824(pASspo) exhibits a rapid increase in butanol production between 16 and 64 hours growth, at which timepoint butanol production remains constant for the remainder of the fermentation. A maximum butanol concentration of ˜153 mM was recorded in 824(pASspo), which is a 132% increase compared to the control strain.

By decreasing SPOIIE activity using an antisense oligonucleotide expressed from the pASspo plasmid, the Clostridia spent a greater amount of time undergoing solventogenesis, were able to reproduce to a higher density of cells, and inhibit sporulation. The overall effect of reducing SPOIIE activity is a drastic increase in solvent production from engineered solvent producing Clostridia.

EXAMPLE 6

Morphology and Sporulation

Strains harboring pASsos and pASspo were grown simultaneously were observed at 24, 48, 72 and 140 hour intervals. At 24 hours growth, both strains are morphologically similar with cells are visible in all stages of division, and in neither strain are sporulating cells observed. After 48 hours growth, many 824(pASspo) cells can be seen dividing, whereas majority of 824(pASsos) cells are single rods with the occasional sporulating cell. After 72 hours, many 824(pASsos) cells can be seen to be sporulating, but there are still some 824(pASspo) cells that are in the process of division. Additionally, some single cells have an abnormal morphology, such that they are elongated two- to threefold compared to the control. Examination of several different cultures of 824(pASspo) indicated that these elongated cells are common, and that they were not mis-identified as vegetative cells undergoing division. After 140 hours growth, sporulating cells or free endospores dominated the 824(pASsos) culture, with very few vegetative cells observed. In contrast, very few sporulating cells were observed in cultures of 824(pASspo), with the majority of cells appearing to be in the vegetative growth state. Of those cells which were sporulating, there were several types of abnormal morphology that could be observed. These experiments indicate that the antisense DNA was properly expressed, decreased SPOIIE activity, and inhibited, delayed or drastically reduced the cells ability to undergo sporulation.

EXAMPLE 7

SpoIIE-Disrupted Strains

The plasmid pSpoΔ4 was constructed from a fragment of spoIIE (bases 3351731 through 3354118 of the C. acetobutylicum genome, GENBANK® Acc. # NC_(—)003030). DNA spanning from the 509th base to the 1113th base of the open reading frame was amplified by PCR using primers “spofragUP” (SEQ ID NO: 11; containing an EcoRI restriction site) and “spofragDS” (SEQ ID NO: 12; containing an XbaI restriction site). Vector pSA12 and the spoIIE fragment were digested with EcoRI and XbaI, and ligated to form plasmid pPreSpoΔ4. The ˜0. 9 kb catP gene was PCR amplified by from plasmid pIMPTH (16) using primers “catPstN”(SEQ ID NO: 13) and “catPstC” (SEQ ID NO: 14) both primers contain PstI restriction sites. A PstI restriction site was located in the centre of the spoIIE fragment. Vector pPreSpoΔ4 and the catP gene were digested with PstI and ligated to form vector pSpoΔ4. Correct construction of pSpoΔ4 was confirmed by sequencing with primers “spofragUP” (SEQ ID NO: 11) and “spofragDS” (SEQ ID NO: 12). The plasmid pSpoΔ4 was electrotransformed into C. acetobutylicum according to standard protocol. Positive transformants of wild type cells were selected on Em media and transformants of Mutants B, H and buk- selected on Em/Thi media. Single colonies of positive transformants were grown up overnight in CGM supplemented with Em. 20 μl was streaked on RCM plates, and allowed to grow for 48 hours prior to replica plating onto fresh RCM plates. Replica plating was carried out 5 times. Additionally, 20 μl from the original cultures was streaked on CGM containing Em, Thi, and Thi/Em to confirm that the pSpoΔ4 plasmid was not lost from the Em-resistant mutant strains.

A final replica plating was performed to transfer colonies onto CGM supplemented with Thi. 10 colonies of each strain were grown up for further testing. All colonies were tested by purification of the genome and PCR amplification used to confirm both the strain background and the correct insertion of the spoIIE disruption cassette. Genomic DNA was purified using PUREGENE® Genomic DNA Purification Kit from (Gentra Systems, Minneapolis, Minn. ). The MASTERTAQ® PCR kit (EPPENDORF®) was used for all PCRs. TABLE 4 PCR PRODUCT CONFIRMS DISRUPTION Primer 1: SEQ ID NO. Primer 2 SEQ ID NO. Wild-type Mutant product spoORFfor 15 spoORFrev 15 2.4 kb 3.3 kb spoIIE-strain spoORFfor 15 catPstN 13 Null 1.7 kb spoIIE-strain bukDfor 17 bukDrev 18 0.9 kb 5.5 buk-strain solR453 19 Tc238 20 Null 2.1 kb pO1X (Mut B and Mut H)   7 kb MutH solR453 19 solR1361 21 0.9 kb Null Mut B adhEleft 7 adhEright 8 2.9 kb pSOL1 Null = degenerate sinRfor 9 sinRrev 10 Genomic control

Mutants disrupted for spoIIE were identified in all background strains, and were named Mutant S (wild type background, spoIIE disrupted), Mutant BS (Mutant B background, spoIIE disrupted), Mutant HS (Mutant H background, spoIIE disrupted) and Mutant bukS (buk-background, spoIIE disrupted). Additionally, one strain of Mutant S degenerated and this was called Mutant M5S. This strain will be characterized as compared to Mutant S and also M5. C. acetobutylicum strains with disrupted SpoIIE genes provide an ideal strain for continuous fermentation and batch production of solvents. It is expected that the cells harboring a genomic disruption of the spoIIE knockout will provide a more stable cell strain and provide a complete inactivation of the SPOIIE protein. It is also predicted that this will dramatically increase solvent production using these strains.

EXAMPLE 8

SpoIIE-Homologues

The gene designated CAC3205 in C. acetobutylicum has been identified as SpoIIE (28, GENBANK® Acc. # NC_(—)003030). The SPOIIE cDNA and protein can be found at SEQ ID NO: 1 and 2. Phylogenetic analysis of the SPOIIE protein sequences verifies isolation of the SpoIIE sequence and identifies SPOIIE as a target in other solvent producing Clostridia. FIG. 5 shows a phylogenetic tree of C. acetobutylicum SPOIIE and its 11 closest relatives from other bacterial species. The B. subtilis SpoIIE is not the closest relative to SpoIIE in C. acetobutylicum, and as expected, the SpoIIE protein from related Clostridium are more closely related than the B. subtilis protein. Therefore methods performed using the C. acetobutylicum SpoIIE cDNA and protein may be used in other related solvent producing Clostridia.

Although B. subtilis do not undergo solventogenesis, the hydropathy plots in FIG. 6 indicate the two Clostridia and Bacillus SPOIIE proteins do have some similar properties and structures. B. subtilis SPOIIE consists of two distinct regions—an N-terminal hydrophobic region that crosses the membrane 10 times, and the C-terminal, cytoplasmic catalytic domain (9). The superimposed plots for SpoIIE in B. subtilis and C. acetobutylicum indicate similar regions of hydrophobicity and hydrophilicity, suggesting that the N-terminus of SpoIIE in C. acetobutylicum forms a similar membrane 10-spanning region. The C-terminal catalytic domain of SpoIIE in C. acetobutylicum also exhibits conservation of critical amino acids as shown in FIG. 7. The asp-610 and asp-628 residues have been shown to be conserved throughout a range of bacterial and eukaryotic PP2C-like phosphatases, and form a metal ion binding pocket within the active site of human PP2C (9). The two conserved regions surrounding the invariant asp-746, gly-747 and asp-795 have also been identified in SpoIIE homologues and PP2C phosphatases in S. pombe, cow, mouse, human and A. thaliana. Mutation of these invariant residues to alanine also causes a severe decrease in sporulation efficiency in B. subtilis (1, 33). All the invariant amino acids conserved between Bacillus and Clostridial SpoIIE are essential and can be used to inactivate the SPOIIE protein in any number of solventogenic Clostridia.

We have shown that the control of solventogenesis and sporulation can be genetically uncoupled in C. acetobutylicum. In strain 824(pASspo), the absence of SpoIIE causes sporulation to be blocked at stage II. The cell remains in a vegetative state, and this allows solvent production to proceed for longer and for solvents to accumulate more rapidly and to a higher concentration. The characteristic drop in OD600 observed in wild type and control strains of C. acetobutylicum after 48-72 hours as the cells transition from the solventogenic phase to sporulation is notably absent in the fermentations of 824(pASspo). Mutant S (wild type background, spoIIE disrupted), Mutant BS (Mutant B background, spoIIE disrupted), Mutant HS (Mutant H background, spoIIE disrupted) and Mutant bukS (buk- background, spoIIE disrupted) were generated to create stable solvent producing bacteria with complete inactivation of the SpoIIE protein. Similarity between the SpoIIE protein of C. acetobutylicum, B. subtilis, and other Clostridial species indicates that the techniques used in C. acetobutylicum can be applied to other solvent producing Clostridia.

All of the references cited herein are expressly incorporated by reference. References are listed again here for convenience:

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1. A method for producing organic solvents comprising: a) culturing said strain under conditions suitable for solventogenesis to generate a culture media; b) reducing SpoIIE activity in a solvent producing strain of Clostridium; and c) purifying solvents from said culture media.
 2. The method of claim 1, wherein said SpoIIE activity is reduced by an antisense oligonucleotide.
 3. The method of claim 2, wherein said antisense oligonucleotide is expressed from a plasmid.
 4. The method of claim 2, wherein said antisense oligonucleotide comprises a nucleotide sequence selected from the group consisting of SEQ ID NO: 22, 23, 24, and
 25. 5. The method of claim 1, wherein SpoIIE activity is reduced by disruption of the SpoIIE gene.
 6. The method of claim 5, wherein said disruption is selected from the group consisting of a mutation, deletion, and interruption of the SpoIIE gene.
 7. A recombinant solvent producing Clostridium having reduced SpoIIE activity sufficient to inhibit sporulation.
 8. The solvent producing Clostridium of claim 7, wherein said SpoIIE activity is reduced by an antisense oligonucleotide.
 9. The solvent producing Clostridium of claim 8, wherein said antisense oligonucleotide is expressed from a plasmid.
 10. The solvent producing Clostridium of claim 9, wherein said plasmid is pASspo.
 11. The solvent producing Clostridium of claim 8, wherein said antisense oligonucleotide comprises a nucleotide sequence selected from the group consisting of SEQ ID NO: 22, 23, 24, and 25
 12. The solvent producing Clostridium of claim 7, wherein said solvent producing Clostridium is selected from the group consisting of Mutant B, Mutant H, Mutant buk-, acetobutylicum, and acetobutylicum ATCC
 824. 13. The solvent producing Clostridium strain of claim 12, selected from the group consisting of 824(pASspo), SK(pASspo), Mutant B (pASspo), Mutant H (pASspo), and Mutant buk-(pASspo).
 14. The solvent producing Clostridium strain of claim 7, wherein said SpoIIE acitivity is reduced by genomic disruption.
 14. The solvent producing Clostridium strain of claim 7, wherein said SpoIIE acitivity is reduced by genomic disruption.
 15. The solvent producing Clostridium strain of claim 7, wherein said strain is Mutant S, Mutant BS, Mutant HS and Mutant bukS.
 16. The solvent producing Clostridium strain of claim 7, wherein said disruption is selected from the group consisting of a mutation, deletion, and interruption of the SpoIIE gene.
 17. The solvent producing Clostridium strain of claim 7, wherein said disruption is constructed from SpoIIE of SEQ ID NO:
 1. 18. The solvent producing Clostridium strain of claim 7, wherein said disruption is mutation of a conserved SpoIIE residue.
 19. The solvent producing Clostridium strain of claim 18, wherein said disruption is mutation of a conserved residue selected from the group consisting of asp-610, asp-628, asp-746, gly-747 and asp-795.
 20. An antisense oligonucleotide comprising a nucleotide sequence selected from the group consisting of SEQ ID NO: 22, 23, 24, and
 25. 